ABSTRACT
Tight junctions are cell-adhesion complexes that seal tissues and are involved in cell polarity and signaling. Supra-molecular assembly and positioning of tight junctions as continuous networks of adhesion strands are dependent on the membrane-associated scaffolding proteins ZO1 and ZO2. To understand how zona occludens (ZO) proteins organize junction assembly, we performed quantitative cell biology and in vitro reconstitution experiments. We discovered that ZO proteins self-organize membrane-attached compartments via phase separation. We identified the multivalent interactions of the conserved PDZ-SH3-GuK supra-domain as the driver of phase separation. These interactions are regulated by phosphorylation and intra-molecular binding. Formation of condensed ZO protein compartments is sufficient to specifically enrich and localize tight-junction proteins, including adhesion receptors, cytoskeletal adapters, and transcription factors. Our results suggest that an active-phase transition of ZO proteins into a condensed membrane-bound compartment drives claudin polymerization and coalescence of a continuous tight-junction belt.
Subject(s)
Tight Junctions/genetics , Zonula Occludens Proteins/genetics , Zonula Occludens-1 Protein/genetics , Zonula Occludens-2 Protein/genetics , Animals , Binding Sites/genetics , Cell Adhesion/genetics , Cell Polarity/genetics , Dogs , HEK293 Cells , Humans , Madin Darby Canine Kidney Cells , Membrane Proteins/genetics , PDZ Domains/genetics , Phosphoproteins/genetics , Phosphorylation/genetics , Protein Binding/genetics , Signal Transduction/genetics , Tight Junctions/metabolism , Zonula Occludens Proteins/chemistry , Zonula Occludens Proteins/ultrastructure , Zonula Occludens-1 Protein/chemistry , Zonula Occludens-1 Protein/ultrastructure , Zonula Occludens-2 Protein/chemistry , Zonula Occludens-2 Protein/ultrastructure , src Homology Domains/geneticsABSTRACT
Stimulated emission depletion (STED) microscopy is routinely used to resolve the ultrastructure of cells with a â¼10-fold higher resolution compared to diffraction limited imaging. While STED microscopy is based on preparing the excited state of fluorescent probes with light, the recently developed expansion microscopy (ExM) provides subdiffraction resolution by physically enlarging the sample before microscopy. The expansion of the fixed cells by cross-linking and swelling of hydrogels easily enlarges the sample â¼4-fold and hence increases the effective optical resolution by this factor. To overcome the current limits of these complementary approaches, we combined ExM with STED (ExSTED) and demonstrated an increase in resolution of up to 30-fold compared to conventional microscopy (<10 nm lateral and â¼50 nm isotropic). While the increase in resolution is straightforward, we found that high-fidelity labeling via multi-epitopes is required to obtain emitter densities that allow ultrastructural details with ExSTED to be resolved. Our work provides a robust template for super-resolution microscopy of entire cells in the ten nanometer range.
ABSTRACT
Quantifying molecular dynamics of cell membrane constituents is required to understand organization and function of biological membranes. Because of its complex structure unambiguous interpretation of molecular membrane dynamics requires high spatial and temporal resolution measurements. In this paper, we provide a comprehensive description of circle scanning fluorescence correlation spectroscopy and its combination with stimulated emission depletion microscopy (CS-STED-FCS). This method allows quantification of sub-diffusion processes and direct mapping of heterogeneities in membranes with high spatiotemporal resolution. We show how to use model membranes to calibrate and test the technique and how to apply it in the context of living cells to quantify membrane dynamics with high spatiotemporal resolution and good statistics.
Subject(s)
Cell Membrane/metabolism , Image Processing, Computer-Assisted/methods , Intravital Microscopy/methods , Spectrometry, Fluorescence/methods , Animals , Calibration , Cell Line , Diffusion , Fluorescent Dyes/chemistry , Humans , Intravital Microscopy/instrumentation , Lipid Bilayers/metabolism , Membrane Proteins/metabolism , Microscopy, Fluorescence/instrumentation , Microscopy, Fluorescence/methods , Molecular Dynamics Simulation , Spectrometry, Fluorescence/instrumentationABSTRACT
The spatiotemporal organization of cytokine receptors in the plasma membrane is still debated with models ranging from ligand-independent receptor pre-dimerization to ligand-induced receptor dimerization occurring only after receptor uptake into endosomes. Here, we explore the molecular and cellular determinants governing the assembly of the type II interleukin-4 receptor, taking advantage of various agonists binding the receptor subunits with different affinities and rate constants. Quantitative kinetic studies using artificial membranes confirm that receptor dimerization is governed by the two-dimensional ligand-receptor interactions and identify a critical role of the transmembrane domain in receptor dimerization. Single molecule localization microscopy at physiological cell surface expression levels, however, reveals efficient ligand-induced receptor dimerization by all ligands, largely independent of receptor binding affinities, in line with the similar STAT6 activation potencies observed for all IL-4 variants. Detailed spatiotemporal analyses suggest that kinetic trapping of receptor dimers in actin-dependent microcompartments sustains robust receptor dimerization and signalling.
Subject(s)
Cell Membrane/metabolism , Receptors, Interleukin-4, Type II/metabolism , Actin Cytoskeleton , Cell Compartmentation , Dimerization , HeLa Cells , Humans , Ligands , Receptors, Interleukin-4, Type II/agonists , STAT6 Transcription Factor/metabolismABSTRACT
FGF2 is secreted from cells by an unconventional secretory pathway. This process is mediated by direct translocation across the plasma membrane. Here, we define the minimal molecular machinery required for FGF2 membrane translocation in a fully reconstituted inside-out vesicle system. FGF2 membrane translocation is thermodynamically driven by PI(4,5)P2-induced membrane insertion of FGF2 oligomers. The latter serve as dynamic translocation intermediates of FGF2 with a subunit number in the range of 8-12 FGF2 molecules. Vectorial translocation of FGF2 across the membrane is governed by sequential and mutually exclusive interactions with PI(4,5)P2 and heparan sulfates on opposing sides of the membrane. Based on atomistic molecular dynamics simulations, we propose a mechanism that drives PI(4,5)P2 dependent oligomerization of FGF2. Our combined findings establish a novel type of self-sustained protein translocation across membranes revealing the molecular basis of the unconventional secretory pathway of FGF2.
Subject(s)
Fibroblast Growth Factor 2/metabolism , Membrane Transport Proteins/metabolism , Protein Multimerization , Secretory Vesicles/metabolism , Heparitin Sulfate/metabolism , Molecular Dynamics Simulation , Phosphatidylinositol 4,5-Diphosphate/metabolismABSTRACT
A deregulation of ceramide biosynthesis in the endoplasmic reticulum (ER) is frequently linked to induction of mitochondrial apoptosis. Although in vitro studies suggest that ceramides might initiate cell death by acting directly on mitochondria, their actual contribution to the apoptotic response in living cells is unclear. Here, we have analyzed the consequences of targeting the biosynthetic flow of ceramides to mitochondria using a ceramide transfer protein (encoded by COL4A3BP) equipped with an OMM anchor, mitoCERT. Cells expressing mitoCERT import ceramides into mitochondria and undergo Bax-dependent apoptosis. Apoptosis induction by mitoCERT was abolished through (i) removal of its ceramide transfer domain, (ii) disruption of its interaction with VAMP-associated proteins (VAPs) in the ER, (iii) addition of antagonistic CERT inhibitor HPA12, (iv) blocking de novo ceramide synthesis and (v) targeting of a bacterial ceramidase to mitochondria. Our data provide the first demonstration that translocation of ER ceramides to mitochondria specifically commits cells to death and establish mitoCERT as a valuable new tool to unravel the molecular principles underlying ceramide-mediated apoptosis.
Subject(s)
Apoptosis , Ceramides/metabolism , Mitochondria/metabolism , Protein Serine-Threonine Kinases/metabolism , bcl-2-Associated X Protein/metabolism , Biocatalysis , Biological Transport , Endoplasmic Reticulum/metabolism , HeLa Cells , Humans , Protein Binding , Protein Transport , Vesicular Transport Proteins/metabolism , bcl-2 Homologous Antagonist-Killer Protein/metabolismABSTRACT
The investigation of the subcellular localization, dynamics and interaction of proteins and protein complexes in prokaryotes is complicated by the small size of the cells. Super-resolution microscopy (SRM) comprise various new techniques that allow light microscopy with a resolution that can be up to ten-fold higher than conventional light microscopy. Application of SRM techniques to living prokaryotes demands the introduction of suitable fluorescent probes, usually by fusion of proteins of interest to fluorescent proteins with properties compatible to SRM. Here we describe an approach that is based on the genetically encoded self-labelling enzymes HaloTag and SNAP-tag. Proteins of interest are fused to HaloTag or SNAP-tag and cell permeable substrates can be labelled with various SRM-compatible fluorochromes. Fusions of the enzyme tags to subunits of a type I secretion system (T1SS), a T3SS, the flagellar rotor and a transcription factor were generated and analysed in living Salmonella enterica. The new approach is versatile in tagging proteins of interest in bacterial cells and allows to determine the number, relative subcellular localization and dynamics of protein complexes in living cells.
Subject(s)
Bacterial Proteins/metabolism , Bacterial Secretion Systems/metabolism , Fluorescent Dyes/metabolism , Molecular Imaging/methods , Salmonella enterica/enzymology , Staining and Labeling/methods , Bacterial Proteins/genetics , Bacterial Secretion Systems/genetics , Fluorescent Dyes/pharmacology , Recombinant Fusion Proteins/genetics , Recombinant Fusion Proteins/metabolism , Salmonella enterica/cytology , Salmonella enterica/geneticsABSTRACT
We present an ultrasensitive technique for quantitative protein-protein interaction analysis in a two-dimensional format based on phase-separated, micropatterned membranes. Interactions between proteins captured to lipid probes via an affinity tag trigger partitioning into the liquid-ordered phase, which is readily quantified by fluorescence imaging. Based on a calibration with well-defined low-affinity protein-protein interactions, equilibrium dissociation constants >1 mM were quantified. Direct capturing of proteins from mammalian cell lysates enabled us to detect homo- and heterodimerization of signal transducer and activator of transcription proteins. Using the epidermal growth factor receptor (EGFR) as a model system, quantification of low-affinity interactions between different receptor domains contributing to EGFR dimerization was achieved. By exploitation of specific features of the membrane-based assay, the regulation of EGFR dimerization by lipids was demonstrated.
Subject(s)
ErbB Receptors/metabolism , Lipids/chemistry , Membranes, Artificial , Optical Imaging/instrumentation , Protein Interaction Mapping/instrumentation , Animals , Equipment Design , ErbB Receptors/analysis , Humans , Microscopy, Fluorescence/instrumentation , Microscopy, Fluorescence/methods , Models, Molecular , Optical Imaging/methods , Phase Transition , Protein Interaction Mapping/methods , Protein Interaction Maps , Protein Multimerization , Signal TransductionABSTRACT
Type I interferons (IFNs) activate differential cellular responses through a shared cell surface receptor composed of the two subunits, IFNAR1 and IFNAR2. We propose here a mechanistic model for how IFN receptor plasticity is regulated on the level of receptor dimerization. Quantitative single-molecule imaging of receptor assembly in the plasma membrane of living cells clearly identified IFN-induced dimerization of IFNAR1 and IFNAR2. The negative feedback regulator ubiquitin-specific protease 18 (USP18) potently interferes with the recruitment of IFNAR1 into the ternary complex, probably by impeding complex stabilization related to the associated Janus kinases. Thus, the responsiveness to IFNα2 is potently down-regulated after the first wave of gene induction, while IFNß, due to its â¼100-fold higher binding affinity, is still able to efficiently recruit IFNAR1. Consistent with functional data, this novel regulatory mechanism at the level of receptor assembly explains how signaling by IFNß is maintained over longer times compared with IFNα2 as a temporally encoded cause of functional receptor plasticity.
Subject(s)
Endopeptidases/metabolism , Interferon Type I/physiology , Receptor, Interferon alpha-beta/metabolism , HeLa Cells , Humans , Janus Kinase 1/metabolism , Protein Binding , Protein Multimerization , Protein Stability , Signal Transduction , Ubiquitin ThiolesteraseABSTRACT
Interactions of proteins in the plasma membrane are notoriously challenging to study under physiological conditions. We report in this paper a generic approach for spatial organization of plasma membrane proteins into micropatterns as a tool for visualizing and quantifying interactions with extracellular, intracellular, and transmembrane proteins in live cells. Based on a protein-repellent poly(ethylene glycol) polymer brush, micropatterned surface functionalization with the HaloTag ligand for capturing HaloTag fusion proteins and RGD peptides promoting cell adhesion was devised. Efficient micropatterning of the type I interferon (IFN) receptor subunit IFNAR2 fused to the HaloTag was achieved, and highly specific IFN binding to the receptor was detected. The dynamics of this interaction could be quantified on the single molecule level, and IFN-induced receptor dimerization in micropatterns could be monitored. Assembly of active signaling complexes was confirmed by immunostaining of phosphorylated Janus family kinases, and the interaction dynamics of cytosolic effector proteins recruited to the receptor complex were unambiguously quantified by fluorescence recovery after photobleaching.
Subject(s)
Cell Membrane/metabolism , Endopeptidases/metabolism , Fluorescence Recovery After Photobleaching , Green Fluorescent Proteins/metabolism , HeLa Cells , Humans , Janus Kinase 1/metabolism , Protein Binding , Protein Multimerization , Protein Transport , Receptor, Interferon alpha-beta/metabolism , Recombinant Fusion Proteins/metabolism , STAT2 Transcription Factor/metabolism , Signal Transduction , Single-Cell Analysis , TYK2 Kinase/metabolism , Time-Lapse Imaging , Ubiquitin ThiolesteraseABSTRACT
The microtubule-associated phosphoprotein tau regulates microtubule dynamics and is involved in neurodegenerative diseases collectively called tauopathies. It is generally believed that the vast majority of tau molecules decorate axonal microtubules, thereby stabilizing them. However, it is an open question how tau can regulate microtubule dynamics without impeding microtubule-dependent transport and how tau is also available for interactions other than those with microtubules. Here we address this apparent paradox by fast single-molecule tracking of tau in living neurons and Monte Carlo simulations of tau dynamics. We find that tau dwells on a single microtubule for an unexpectedly short time of â¼40 ms before it hops to the next. This dwell time is 100-fold shorter than previously reported by ensemble measurements. Furthermore, we observed by quantitative imaging using fluorescence decay after photoactivation recordings of photoactivatable GFP-tagged tubulin that, despite this rapid dynamics, tau is capable of regulating the tubulin-microtubule balance. This indicates that tau's dwell time on microtubules is sufficiently long to influence the lifetime of a tubulin subunit in a GTP cap. Our data imply a novel kiss-and-hop mechanism by which tau promotes neuronal microtubule assembly. The rapid kiss-and-hop interaction explains why tau, although binding to microtubules, does not interfere with axonal transport.
Subject(s)
Axons/metabolism , Microtubules/metabolism , Signal Transduction/genetics , Tubulin/metabolism , tau Proteins/metabolism , Animals , Axonal Transport , Cell Differentiation , Gene Expression , Genes, Reporter , Genetic Vectors , Green Fluorescent Proteins/genetics , Green Fluorescent Proteins/metabolism , Kinetics , Lentivirus/genetics , Microscopy, Fluorescence , Microtubules/chemistry , Microtubules/ultrastructure , Molecular Dynamics Simulation , Molecular Imaging , Monte Carlo Method , PC12 Cells , Rats , Tubulin/chemistry , tau Proteins/geneticsABSTRACT
Lipid analogues carrying three nitrilotriacetic acid (tris-NTA) head groups were developed for the selective targeting of His-tagged proteins into liquid ordered (lo ) or liquid disordered (ld ) lipid phases. Strong partitioning into the lo phase of His-tagged proteins bound to tris-NTA conjugated to saturated alkyl chains (tris-NTA DODA) was achieved, while tris-NTA conjugated to an unsaturated alkyl chain (tris-NTA SOA) predominantly resided in the ld phase. Interestingly, His-tag-mediated lipid crosslinking turned out to be required for efficient targeting into the lo phase by tris-NTA DODA. Robust partitioning into lo phases was confirmed by using viral lipid mixtures and giant plasma membrane vesicles. Moreover, efficient protein targeting into lo and ld domains within the plasma membrane of living cells was demonstrated by single-molecule tracking, thus establishing a highly generic approach for exploring lipid microdomains inâ situ.
Subject(s)
Acetates/chemistry , Membrane Microdomains/metabolism , Nitro Compounds/metabolism , Proteins/metabolism , Diffusion , HeLa Cells , Histidine/chemistry , Histidine/genetics , Histidine/metabolism , Humans , Maltose-Binding Proteins/chemistry , Maltose-Binding Proteins/genetics , Maltose-Binding Proteins/metabolism , Membrane Microdomains/chemistry , Nitrilotriacetic Acid/chemistry , Nitro Compounds/chemistry , Oligopeptides/chemistry , Oligopeptides/genetics , Oligopeptides/metabolism , Protein Binding , Proteins/chemistry , Recombinant Fusion Proteins/biosynthesis , Recombinant Fusion Proteins/chemistry , Recombinant Fusion Proteins/genetics , Unilamellar Liposomes/chemistry , Unilamellar Liposomes/metabolismABSTRACT
We have established an approach for the spatial control of lipid phase separation in tethered polymer-supported membranes (PSMs), which were obtained by vesicle fusion on a poly(ethylene glycol) polymer brush functionalized with fatty acid moieties. Phase separation of ternary lipid mixtures (1,2-dioleoyl-sn-glycero-3-phosphocholine/sphingomyelin/cholesterol) into liquid-disordered (l(d)) and liquid-ordered (l(o)) phases within both leaflets was obtained with palmitic acid as the anchoring group. In contrast, tethering of the PSM with oleic acid interfered with the phase separation in the surface-proximal leaflet. We exploited this feature for the assembly of l(o) domains within PSMs into defined structures by binary micropatterning of palmitic and oleic acid into complementary areas. Ternary lipid mixtures spontaneously separated into l(o) and l(d) phases controlled by the geometry of the underlying tethers. Transmembrane proteins reconstituted in these phase-separated PSMs strictly partitioned into the l(d) phase. Hence, the l(o) phase could be used for confining transmembrane proteins into microscopic and submicroscopic domains.
Subject(s)
Lipid Bilayers/chemistry , Lipids/chemistry , Membrane Proteins/chemistry , Polyethylene Glycols/chemistry , Diffusion , Particle Size , Surface PropertiesABSTRACT
Quantum dots (QD) are powerful labels for probing diffusion and interaction dynamics of proteins on the single molecule level in living cells. Protein cross-linking due to multifunctional QD strongly affects these properties. This becomes particularly critical when labeling interaction partners with QDs for interrogating the dynamics of complexes. We have here implemented a generic method for QD monofunctionalization based on electrostatic repulsion of a highly negatively charged peptide carrier. On the basis of this method, monobiotinylated QDs were prepared with high yield as confirmed by single molecule assays. These QDs were successfully employed for probing the assembly and diffusion dynamics of binary and ternary cytokine-receptor complexes on the surface of living cells by dual color single QD tracking. Thus, sequential and dynamic recruitment of the type I interferon receptor subunits by the ligand could be observed.
Subject(s)
Multiprotein Complexes/metabolism , Quantum Dots , Receptor, Interferon alpha-beta/metabolism , Static Electricity , HeLa Cells , Humans , Models, Biological , Molecular Structure , Multiprotein Complexes/chemistry , Receptor, Interferon alpha-beta/chemistryABSTRACT
In living color: efficient intracellular covalent labeling of proteins with a photoswitchable dye using the HaloTag for dSTORM super-resolution imaging in live cells is described. The dynamics of cellular nanostructures at the plasma membrane were monitored with a time resolution of a few seconds. In combination with dual-color FPALM imaging, submicroscopic receptor organization within the context of the membrane skeleton was resolved.
Subject(s)
Cell Membrane/chemistry , Green Fluorescent Proteins/chemistry , Microscopy, Fluorescence/methods , Actins/chemistry , Actins/metabolism , Cell Membrane/metabolism , Cytoskeleton/chemistry , Cytoskeleton/metabolism , Fluorescent Dyes/chemistry , Green Fluorescent Proteins/metabolism , HeLa Cells , Humans , Nanostructures/chemistry , TransfectionABSTRACT
Spatial organization of proteins into microscopic structures has important applications in fundamental and applied research. Preserving the function of proteins in such microstructures requires generic methods for site-specific capturing through affinity handles. Here, we present a versatile bottom-up surface micropatterning approach based on surface functionalization with maleimides, which selectively react with organic thiols. Upon UV irradiation through a photomask, the functionality of illuminated maleimide groups was efficiently destroyed. Remaining maleimides in nonilluminated regions were further reacted with different thiol-functionalized groups for site-specific protein immobilization under physiological conditions. Highly selective immobilization of His-tagged proteins into tris(nitrilotriacetic acid) functionalized microstructures with very high contrast was possible even by direct capturing of proteins from crude cell lysates. Moreover, we employed phosphopantetheinyl transfer from surface-immobilized coenzyme A to ybbR-tagged proteins in order to implement site-specific, covalent protein immobilization into microstructures. The functional integrity of the immobilized protein was confirmed by monitoring protein-protein interactions in real time. Moreover, we demonstrate quantitative single-molecule analysis of protein-protein interactions with proteins selectively captured into these high-contrast micropatterns.
Subject(s)
Maleimides/chemistry , Protein Interaction Mapping , Proteins/chemistry , Coenzyme A/chemistry , Green Fluorescent Proteins/chemistry , Green Fluorescent Proteins/genetics , Green Fluorescent Proteins/metabolism , Histidine/chemistry , Histidine/genetics , Histidine/metabolism , Immobilized Proteins/chemistry , Interferon-alpha/chemistry , Oligopeptides/chemistry , Oligopeptides/genetics , Oligopeptides/metabolism , Protein Binding , Spectrometry, Fluorescence , Sulfhydryl Compounds/chemistry , Surface PropertiesABSTRACT
Fluorescent probes for biological imaging of single molecules (SM) have many stringent design requirements. In the case of quantum dot (QD) probes, it remains a challenge to control their functional properties with high precision. Here, we describe the simple preparation of QDs with reduced size and monovalency. Our approach combines a peptide surface coating, stable covalent conjugation of targeting units and purification by gel electrophoresis. We precisely characterize these probes by ensemble and SM techniques and apply them to tracking individual proteins in living cells.
